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通过表面等离子体荧光光谱法研究的DNA-DNA杂交动力学的匹配碱基对数依赖性。

Matching base-pair number dependence of the kinetics of DNA-DNA hybridization studied by surface plasmon fluorescence spectroscopy.

作者信息

Tawa Keiko, Yao Danfeng, Knoll Wolfgang

机构信息

Max-Planck-Institute for Polymer Research, Ackermannweg 10, D-55128 Mainz, Germany.

出版信息

Biosens Bioelectron. 2005 Aug 15;21(2):322-9. doi: 10.1016/j.bios.2004.10.024. Epub 2004 Dec 8.

Abstract

Two single-stranded DNA oligonucleotides consisting of complementary base-pairs can form double strands. This phenomenon is well studied in solutions, however, in order to clarify the physical mechanism of the hybridization occurring at a solid/solution interface, we studied the kinetics by surface plasmon fluorescence spectroscopy (SPFS): one single-stranded oligo-DNA (probe-DNA) was immobilized on the substrate, the other one (target-DNA) labelled with a fluorescent probe was added to the flow cell. After hybridization, the chromophores could be excited by the surface plasmon mode and their fluorescence detected with high sensitivity. The dependence of the k(on) and k(off) rate constants on the length of the hybridizing oligonucleotides was investigated by using a MM0 series (no mismatch) and the kinetics was found to be well described by a Langmuir adsorption model. From these measurements we found that also in the case of surface hybridization the affinity of the duplexes decreases as the number of matching base-pairs decreases from 15 to 10. In order to show that SPFS is the powerful technique with high sensitivity, the hybridization process for mixed target-oligos was measured by SPFS and analyzed by an expanded Langmuir model in which two components of target-oligo can bind to probe-DNA at the sensor surface competitively. Two sets of the k(on) and k(off) obtained from the experiment are successfully consistent with the k(on) and k(off) obtained from experiments for single (pure) target-DNA.

摘要

由互补碱基对组成的两条单链DNA寡核苷酸可以形成双链。这种现象在溶液中已得到充分研究,然而,为了阐明在固/液界面发生杂交的物理机制,我们通过表面等离子体荧光光谱法(SPFS)研究了动力学:一条单链寡聚DNA(探针DNA)固定在基底上,另一条用荧光探针标记的(靶标DNA)被添加到流通池中。杂交后,发色团可被表面等离子体模式激发,并能高灵敏度地检测到它们的荧光。通过使用MM0系列(无错配)研究了k(on)和k(off)速率常数对杂交寡核苷酸长度的依赖性,发现动力学可以用朗缪尔吸附模型很好地描述。从这些测量中我们发现,在表面杂交的情况下,随着匹配碱基对的数量从15减少到{10},双链体的亲和力也会降低。为了表明SPFS是一种具有高灵敏度的强大技术,通过SPFS测量了混合靶标寡核苷酸的杂交过程,并通过扩展的朗缪尔模型进行分析,在该模型中,靶标寡核苷酸的两个组分可以在传感器表面竞争性地与探针DNA结合。从实验中获得的两组k(on)和k(off)与从单一(纯)靶标DNA实验中获得的k(on)和k(off)成功一致。

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